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W tym Artykule

  • Podsumowanie
  • Streszczenie
  • Wprowadzenie
  • Protokół
  • Wyniki
  • Dyskusje
  • Ujawnienia
  • Podziękowania
  • Materiały
  • Odniesienia
  • Przedruki i uprawnienia

Podsumowanie

An in vivo physiological model of α-synuclein is required to study and understand the pathogenesis of Parkinson's disease. We describe a method to monitor the cytotoxicity and aggregate formation of α-synuclein using a humanized yeast model.

Streszczenie

Parkinson's disease is the second most common neurodegenerative disorder and is characterized by progressive cell death caused by the formation of Lewy bodies containing misfolded and aggregated α-synuclein. α-synuclein is an abundant presynaptic protein that regulates synaptic vesicle trafficking, but the accumulation of its proteinaceous inclusions results in neurotoxicity. Recent studies have revealed that various genetic factors, including bacterial chaperones, could reduce the formation of α-synuclein aggregates in vitro. However, it is also important to monitor the anti-aggregation effect in the cell to apply this as a potential treatment for the patients. It would be ideal to use neuronal cells, but these cells are difficult to handle and take a long time to exhibit the anti-aggregation phenotype. Therefore, a quick and effective in vivo tool is required for the further evaluation of in vivo anti-aggregation activity. The method described here was used to monitor and analyze the anti-aggregation phenotype in the humanized yeast Saccharomyces cerevisiae, which expressed human α-synuclein. This protocol demonstrates in vivo tools that could be used for monitoring α-synuclein-induced cellular toxicity, as well as the formation of α-synuclein aggregates in cells.

Wprowadzenie

Parkinson's disease (PD) is a serious problem for aging societies worldwide. The aggregation of α-synuclein is closely associated with PD, and protein aggregates of α-synuclein are widely used as a molecular biomarker for diagnosing the disease1. α-synuclein is a small acidic protein (140 amino acids in length) with three domains, namely the N-terminal lipid-binding α-helix, the amyloid-binding central domain (NAC), and the C-terminal acidic tail2. The misfolding of α-synuclein can occur spontaneously and eventually leads to the formation of amyloid aggregates called Lewy bodies3. α-synuclein may contribute to the pathogenesis of PD in several ways. In general, it is thought that its abnormal, soluble oligomeric forms called protofibrils are toxic species that cause neuronal cell death by affecting various cellular targets, including synaptic function3.

The biological models used to study neurodegenerative diseases must be relevant to humans with respect to their genome and cellular biology. The best models would be human neuronal cell lines. However, these cell lines are associated with several technical issues, such as difficulties in the maintenance of cultures, low efficiency of transfection, and high expense4. For these reasons, an easy and reliable tool is required to accelerate the progress in this research area. Importantly, the tool should be easy to use for analyzing the collected data. From these perspectives, various model organisms have been widely used, including Drosophila, Caenorhabditis elegans, Danio rerio, yeast, and rodents5. Among them, yeast is the best model organism because genetic manipulation is easy, and it is cheaper than the other model organisms. Most importantly, yeast has high similarities to human cells, such as 60% sequence homology to human orthologs and 25% close homology with human disease-related genes6, and they also share fundamental eukaryotic cell biology. Yeast contains many proteins with similar sequences and analogous functions to those in human cells7. Indeed, yeast expressing human genes has been widely used as a model system to elucidate cellular processes8. This yeast strain is called humanized yeast and is a useful tool for exploring the function of human genes9. Humanized yeast has merit for studying genetic interactions because genetic manipulation is well established in yeast.

In this study, we used the yeast Saccharomyces cerevisiae as a model organism to study the pathogenesis of PD, particularly for investigating α-synuclein aggregate formation and cytotoxicity10. For the expression of α-synuclein in the budding yeast, the W303a strain was used for transformation with plasmids encoding for the wild-type and familial PD-associated variants of α-synuclein. As the W303a strain has an auxotrophic mutation on URA3, it is applicable for the selection of cells containing plasmids with URA3. The expression of α-synuclein encoded in a plasmid is regulated under the GAL1 promoter. Thus, the expression level of α-synuclein can be controlled. In addition, the fusion of green fluorescent protein (GFP) at the C-terminal region of α-synuclein allows the monitoring of α-synuclein foci formation. To understand the characteristics of the familial PD-associated variants of α-synuclein, we also expressed these variants in yeast and examined their cellular effects. This system is a straightforward tool for screening compounds or genes exhibiting protective roles against the cytotoxicity of α-synuclein.

Protokół

1. Preparation of media and solutions

  1. Media preparation
    1. To prepare YPD medium, dissolve 50 g of YPD powder in dH2O to make a final volume of 1 L. Autoclave for sterilization. Store at room temperature (RT).
    2. To make YPD agar medium, dissolve 50 g of YPD powder and 20 g of agar in 1 L of dH2O. Autoclave for sterilization. After cooling down, pour onto Petri dishes. Store at 4 ˚C.
    3. To make SC with raffinose (SRd)-Ura medium, dissolve 6.7 g of yeast nitrogen base with ammonium sulfate and without amino acids in 795 mL of dH2O. Autoclave for sterilization. Add 100 mL of 20% raffinose, 5 mL of 20% glucose, and 100 mL of 10x -Ura drop-out before use.
    4. To make SD-Ura agar medium, dissolve 6.7 g of yeast nitrogen base with ammonium sulfate and without amino acids and 20 g of agar in 800 mL of dH2O. Autoclave in a flask with a volume over 2 L. Add 100 mL of 20% glucose and 100 mL of 10x -Ura drop-out. Mix well and pour onto Petri dishes. Store at 4 ˚C.
    5. To make SC with galactose (SG)-Ura agar medium, dissolve 6.7 g of yeast nitrogen base with ammonium sulfate and without amino acids and 20 g of agar in 800 mL of dH2O. Autoclave in a flask with a volume over 2 L. Add 100 mL of 20% galactose and 100 mL of 10x -Ura drop-out. Mix well and pour on Petri dishes. Store at 4 ˚C.
  2. Stock solutions to use with SD media
    1. To make a 20% carbon source (glucose, galactose, and raffinose), dissolve 100 g of glucose, galactose, or raffinose in dH2O to make a final volume of 500 mL. Autoclave and store at RT.
    2. To make 10x yeast synthetic drop-out medium supplements without uracil (10x-Ura drop-out), dissolve 19.2 g of "yeast synthetic drop-out medium supplements without uracil" in dH2O to make a final volume of 1 L. Autoclave and store at RT.
      ​NOTE: For the preparation of a medium containing agar, add a magnetic stir bar to the flask to mix all the solutions well before pouring onto Petri dishes.

2. Yeast transformation

NOTE: The pRS426 plasmid was used to clone the α-synuclein gene and contained the URA3 gene as a selectable marker. There are familial PD-associated variants of α-synuclein that have severe disease phenotypes (e.g., cytotoxicity). These variants were also used here to monitor their cytotoxicity and aggregated foci formation. Use the same colony of yeast transformants for all the experiments to get consistent results.

  1. For the transformation of the yeast expression plasmids, use an empty vector (pRS426) as the control and α-synuclein-containing plasmids. Referring to the standard lithium acetate (LiAc) method11, prepare six competent cells and 0.5 µg of each plasmid, and perform the transformation.
  2. To select for yeast transformants containing plasmids, use the synthetic defined medium (SD medium) without uracil (SD-Ura), and incubate the plates at 30 ˚C for 2-3 days.
  3. Patch three single colonies onto an SD-Ura agar plate for the selection of cells containing plasmids for further experiments.
    ​NOTE: To generate accurate and reliable results, we examined at least three biological replicates per strain.

3. Spotting assay

NOTE: The expression of GFP-tagged α-synuclein in high-copy number plasmids is known to be associated with cytotoxicity in yeast10.

  1. Inoculate the three patched yeast transformants per strain into 3 mL of SRd-Ura for the selective growth of yeast containing the plasmids with 2% raffinose for inhibition of the induction of α-synuclein under the GAL1 promoter and 0.1% glucose. Incubate the cell culture at 30 °C under agitation at 200 rpm.
    NOTE: Repeating all the experiments with different colonies is important. Obtaining the same results from over three independent colonies means the result is reliable.
  2. The next day, inoculate the overnight cultured cells into 3 mL of fresh SRd-Ura to an OD600 of 0.2, and incubate for 6 h at 30 °C under agitation at 200 rpm. 
  3. When the OD600 reaches 0.6-0.8, dilute the cells in 96-well plates for the spotting assay as follows.
    1. Measure the OD600 of all the samples, and dilute the samples to an OD600 of 0.5 with sterile dH2O (the mixed volume is 100 µL) in lane 1 of a 96-well plate to equalize the number of cells in each culture.
    2. Perform fivefold serial dilutions of the yeast cells by adding 160 µL of sterile dH2O to the next five lanes. Ensure a total volume of 40 µL when serially diluting the cells in each lane.
      NOTE: Low dilution factors can produce larger differences between the samples. Sufficient pipetting is required to ensure uniform mixing when performing the serial dilutions. The pipette tip should be replaced at every dilution point. Otherwise, the cells attached to the surface of the tip could be transferred to the next well and affect the cell number.
  4. Use a multichannel pipette to transfer 10 µL from each well to spot the samples on SD-Ura agar plates for the controls and SG-Ura agar plates to monitor toxicity.
    NOTE: The plates should be dried until the spotted samples are fully absorbed onto the plates.
  5. Incubate the spotted plates upside down at 30 °C for 4 days.
  6. Take images of the plates every 24 h until day 4, and then analyze the data by comparing the growth differences between strains spotted by eye. Count the individual colonies in the most diluted sample, calculate the number of viable cells in the original culture for each strain, or compare the size of the single colonies.

4. Measurement of yeast growth using a microplate reader

  1. Inoculate the three patched yeast transformants per strain into 3 mL of SRd-Ura, and incubate at 30 °C under agitation at 200 rpm overnight.
    NOTE: To understand each colony phenotype of the humanized yeast strain expressing α-synuclein, use the same transformants for all the experiments.
  2. The next day, inoculate the overnight cultured cells into a total of 200 µL of fresh SD-Ura and SG-Ura in 96-well plates. Adjust the final volume, including the cells, to 200 µL, and adjust the initial cell OD600 to 0.05.
    1. Adjust the Program settings in the microtiter plate as follows: set the target temperature to 30 ˚ C, set the shaking (Linear) duration to 890 s, set the shaking (Linear) amplitude to 5 mm, set the interval time to 00:15:00, and set the measurement as absorbance at 600 nm.
    2. Incubate the plate for 2-3 days for all the strains to reach the stationary phase in a microplate reader.
  3. Analyze the data by plotting the growth curve (e.g., using Workbook). Acquire the data points by averaging the values of absorbance from the three biological replicates, and indicate the error bars. Use the value of absorbance from only media as a control, and subtract this from the values from cultured cells (optional).

5. Fluorescence microscopy

  1. Inoculate the patched yeast transformants into 3 mL of SRd-Ura, and culture them overnight at 30 °C under agitation at 200 rpm.
    NOTE: To determine the correlation of the phenotype with the cytotoxicity and foci formation, use the same colonies for the experiment.
  2. The next day, reinoculate the overnight cultured cells into 3 mL of fresh SRd-Ura to an OD600 of 0.003. Incubate the culture until the OD600 reaches 0.2 at 30 °C under agitation at 200 rpm (~18 h).
  3. When an OD600 of 0.2 is achieved, add 300 µL of 20% galactose, and then incubate for another 6 h at 30 °C under agitation at 200 rpm.
  4. Collect the cells by centrifugation at 800 x g for 5 min, and discard the supernatant.
  5. Resuspend the cell pellet gently in 30 µL of distilled water.
  6. Load 5 μL of the resuspended cells onto a slide glass. Prepare an agarose gel pad12 and put it onto the loaded cells to make it spread evenly.
  7. Perform microscopic imaging with a 100x objective using both brightfield and GFP-fluorescence filters.
    1. First, use brightfield to focus the cell with a 100x objective using immersion oil. Use the screen capture option for generating the images using the program.
    2. Switch to a GFP-fluorescence filter. Adjust the image exposure time to between 50 ms and 300 ms to achieve a clear image by balancing the signal-to-noise ratio. Screen capture the image using the program.
    3. Image many cells from multiple points rather than just one.
  8. Analyze the images by counting the percentage of cells containing foci of α-synuclein aggregates using analytical software. Observe the differences between the soluble GFP protein signal and the foci-formed GFP signal, as well as the diffusion of GFP with the A30P variant form of α-synuclein.
    NOTE: Foci formation will be observed with the wild-type, E46K, and A53T variants of α-synuclein. 

Wyniki

The high expression of α-synuclein is known to be linked to neuronal cell death and PD in model systems of PD. This study describes three methods to monitor the cytotoxicity of α-synuclein and the foci formation of aggregated α-synuclein in yeast. Here, the α-synuclein was overexpressed in yeast, and the phenotypes of wild-type α-synuclein and three variants of α-synuclein known as familial mutants of PD were examined (Figure 1 and the Table of Materials...

Dyskusje

Given the complexity of various cellular systems in humans, it is advantageous to use yeast as a model for studying human neurodegenerative diseases. Although it is nearly impossible to investigate the complex cellular interactions of the human brain using yeast, from a single-cell perspective, yeast cells have a high level of similarity to human cells in terms of the genomic sequence homology and fundamental eukaryotic cellular processes8,13. Moreover, given the...

Ujawnienia

The authors have no conflicts of interest to disclose.

Podziękowania

We thank James Bardwell and Tiago F. Outeiro for kindly sharing the plasmids containing α-synuclein. Changhan Lee received funding from the National Research Foundation of Korea (NRF) funded by the Korean government (MSIT) (grant 2021R1C1C1011690), the Basic Science Research Program through the NRF funded by the Ministry of Education (grant 2021R1A6A1A10044950), and the new faculty research fund of Ajou University.

Materiały

NameCompanyCatalog NumberComments
96 well plateSPL30096
AgaroseTAESHIN0158
Bacto AgarBD Difco214010
Breathe-easydiversified biotechBEM-1Gas permeable sealing membrane for microtiter plates
cover glassesMarienfeld24 x 60 mm
Culture tubeSPL40014
Cuvetteratiolab2712120
D-(+)-GalactosesigmaG0625
D-(+)-GlucosesigmaG8270
D-(+)-Raffinose pentahydrateDaejung6638-4105
Incubator (shaking)Labtronmodel: SHI1
Incubator (static)Vision scientificmodel: VS-1203PV-O
LiAcsigmaL6883
Microplate readerTecan30050303 01Model: Infinite 200 pro
multichannel pipette 20-200 µLgilsonFA10011
multichannel pipette 2-20 µLgilsonFA10009
Olympus microscopeOlympusIX-53
PEGsigmaP4338average mol wt 3,350
PetridishSPL10090
pRS426Christianson, T. W., Sikorski, R. S., Dante, M., Shero, J. H. & Hieter, P. Multifunctional yeast high-copy-number shuttle vectors. Gene. 110 (1), 119-122 (1992).
pRS426 GAL1 promoter α-synuclein A30POuteiro, T. F. & Lindquist, S. Yeast cells provide insight into alpha-synuclein biology and pathobiology. Science. 302 (5651), 1772-1775 (2003)
pRS426 GAL1 promoter α-synuclein A53TOuteiro, T. F. & Lindquist, S. Yeast cells provide insight into alpha-synuclein biology and pathobiology. Science. 302 (5651), 1772-1775 (2003)
pRS426 GAL1 promoter α-synuclein E46KOuteiro, T. F. & Lindquist, S. Yeast cells provide insight into alpha-synuclein biology and pathobiology. Science. 302 (5651), 1772-1775 (2003)
pRS426 GAL1 promoter α-synuclein WTOuteiro, T. F. & Lindquist, S. Yeast cells provide insight into alpha-synuclein biology and pathobiology. Science. 302 (5651), 1772-1775 (2003)
ReservoirSPL23050
Spectrophotometereppendorf6131 05560
W303aPresent from James Bardwell
Yeast nitrogen base w/o amino acidsDifco291940
Yeast synthetic drop-out medium supplements without uracilsigmaY1501
YPDCondalab1547.00

Odniesienia

  1. Khurana, V., Lindquist, S. Modelling neurodegeneration in Saccharomyces cerevisiae: Why cook with baker's yeast. Nature Reviews Neuroscience. 11 (6), 436-449 (2010).
  2. Surguchov, A. Intracellular dynamics of synucleins: "Here, there and everywhere". International Review of Cell and Molecular Biology. 320, 103-169 (2015).
  3. Soto, C., Pritzkow, S. Protein misfolding, aggregation, and conformational strains in neurodegenerative diseases. Nature Neuroscience. 21 (10), 1332-1340 (2018).
  4. Gordon, J., Amini, S. General overview of neuronal cell culture. Methods in Molecular Biology. 2311, 1-8 (2021).
  5. Dawson, T. M., Golde, T. E., Lagier-Tourenne, C. Animal models of neurodegenerative diseases. Nature Neuroscience. 21 (10), 1370-1379 (2018).
  6. Bassett, D. E., Boguski, M. S., Hieter, P. Yeast genes and human disease. Nature. 379 (6566), 589-590 (1996).
  7. Koteliansky, V., Glukhova, M., Bejanian, M., Surguchov, A., Smirnov, V. Isolation and characterization of actin-like protein from yeast Saccharomyces cerevisiae. FEBS Letters. 102 (1), 55-58 (1979).
  8. Botstein, D., Chervitz, S. A., Cherry, M. Yeast as a model organism. Science. 277 (5330), 1259-1260 (1997).
  9. Kachroo, A. H., Vandeloo, M., Greco, B. M., Abdullah, M. Humanized yeast to model human biology, disease and evolution. Disease Models & Mechanisms. 15 (6), (2022).
  10. Outeiro, T. F., Lindquist, S. Yeast cells provide insight into alpha-synuclein biology and pathobiology. Science. 302 (5651), 1772-1775 (2003).
  11. Dunham, M., Gartenberg, M., Brown, G. . Methods in Yeast Genetics and Genomics. , (2015).
  12. Skinner, S. O., Sepúlveda, L. A., Xu, H., Golding, I. Measuring mRNA copy number in individual Escherichia coli cells using single-molecule fluorescent in situ hybridization. Nature Protocols. 8 (6), 1100-1113 (2013).
  13. Tenreiro, S., Munder, M. C., Alberti, S., Outeiro, T. F. Harnessing the power of yeast to unravel the molecular basis of neurodegeneration. Journal of Neurochemistry. 127 (4), 438-452 (2013).
  14. Nielsen, J. Yeast systems biology: Model organism and cell factory. Biotechnology Journal. 14 (9), 1800421 (2019).
  15. Eleutherio, E., et al. Oxidative stress and aging: learning from yeast lessons. Fungal Biology. 122 (6), 514-525 (2018).
  16. Rencus-Lazar, S., DeRowe, Y., Adsi, H., Gazit, E., Laor, D. Yeast models for the study of amyloid-associated disorders and development of future therapy. Frontiers in Molecular Biosciences. 6, 15 (2019).
  17. Franco, R., Rivas-Santisteban, R., Navarro, G., Pinna, A., Reyes-Resina, I. Genes implicated in familial Parkinson's disease provide a dual picture of nigral dopaminergic neurodegeneration with mitochondria taking center stage. International Journal of Molecular Sciences. 22 (9), 4643 (2021).
  18. Wan, O. W., Chung, K. K. The role of alpha-synuclein oligomerization and aggregation in cellular and animal models of Parkinson's disease. PLoS One. 7 (6), 38545 (2012).
  19. Xu, L., Pu, J. Alpha-synuclein in Parkinson's disease: From pathogenetic dysfunction to potential clinical application. Parkinson's Disease. 2016, 1720621 (2016).
  20. Gitler, A. D., et al. The Parkinson's disease protein α-synuclein disrupts cellular Rab homeostasis. Proceedings of the National Academy of Sciences of the United States of America. 105 (1), 145-150 (2008).
  21. Sampson, T. R., et al. A gut bacterial amyloid promotes α-synuclein aggregation and motor impairment in mice. Elife. 9, 53111 (2020).
  22. Evans, M. L., et al. The bacterial curli system possesses a potent and selective inhibitor of amyloid formation. Molecular Cell. 57 (3), 445-455 (2015).
  23. Su, L. J., et al. Compounds from an unbiased chemical screen reverse both ER-to-Golgi trafficking defects and mitochondrial dysfunction in Parkinson's disease models. Disease Models & Mechanisms. 3 (3-4), 194-208 (2010).

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Alpha synucleinR pass NucleiHumanized Yeast ModelParkinson s DiseaseCellular PhenotypesGenetic FactorsPlasmidsSD URA Agar PlateSRD URAOptical DensitySpectrophotometerSerial DilutionsToxicity MonitoringYeast Transformants

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